Discovery of a Single-subunit Oligosaccharyltransferase That Enables Glycosylation of Full-length IgG Antibodies in

Overview

Journal bioRxiv

Date 2024 Nov 22

PMID 39574765

Authors

Belen Sotomayor

Thomas C Donahue

Sai Pooja Mahajan

May N Taw

Sophia W Hulbert

Erik J Bidstrup

D Natasha Owitipana

Alexandra Pang

Xu Yang

Souvik Ghosal

Christopher A Alabi

Parastoo Azadi

Jeffrey J Gray

Michael C Jewett

Lai-Xi Wang

Matthew P DeLisa

Affiliations

Soon will be listed here.

Abstract

Human immunoglobulin G (IgG) antibodies are one of the most important classes of biotherapeutic agents and undergo glycosylation at the conserved N297 site in the C2 domain, which is critical for IgG Fc effector functions and anti-inflammatory activity. Hence, technologies for producing authentically glycosylated IgGs are in high demand. While attempts to engineer for this purpose have been described, they have met limited success due in part to the lack of available oligosaccharyltransferase (OST) enzymes that can install linked glycans within the QYNST sequon of the IgG C2 domain. Here, we identified a previously uncharacterized single-subunit OST (ssOST) from the bacterium that exhibited greatly relaxed substrate specificity and, as a result, was able to catalyze glycosylation of native C2 domains in the context of both a hinge-Fc fragment and a full-length IgG. Although the attached glycans were bacterial in origin, conversion to a homogeneous, asialo complex-type G2 -glycan at the QYNST sequon of the -derived hinge-Fc was achieved via chemoenzymatic glycan remodeling. Importantly, the resulting G2-hinge-Fc exhibited strong binding to human FcγRIIIa (CD16a), one of the most potent receptors for eliciting antibody-dependent cellular cytotoxicity (ADCC). Taken together, the discovery of a unique ssOST from provides previously unavailable biocatalytic capabilities to the bacterial glycoprotein engineering toolbox and opens the door to using for the production and glycoengineering of human IgGs and fragments derived thereof.

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